Abstract

The broad objective of this proposal is to understand the interactions of transcriptional regulatory proteins with specific DNA sequence elements and the mechanisms by which these interactions modulate transcription frequency of genes in animal cells. Regulation at this level is critical in determining the developmental fate and function of cells in both normal and disease states. The transcriptional regulation of heat shock genes of Drosophila is to be used as a well-defined and highly-inducible model system. The binding of the heat shock regulatory factor, HSF, to the regulatory elements, HSEs, of heat shock genes is postulated to act catalytically to increase the rate of transcription of adjacent genes. The first section of the grant focuses on binding of HSF to the HSEs, while the second focuses on a potential target for the catalytic action of HSF.
The aims of Section 1 are to investigate the properties and significance of a novel type of protein/DNA interaction between HSF and HSEs. The remarkable flexibility in binding of HSF to different arrangements of a repeated 5 bp recognition unit of HSEs can be explained by recent findings that HSF from induced cells is in the form of a protein trimer. The trimeric nature of HSF has evoked a number of predictions about the structure HSF/HSE complexes that this proposal will test by in vitro binding and interference assays. The biological significance of the strong cooperativity of HSF binding to HSEs observed in vitro will be evaluated by measuring transcription of native and modified heat shock genes using run- on assays of nuclei isolated from transgenic flies.
This aims of Section 2 of the proposal are to investigate the formation and release of the paused (arrested) RNA polymerase II that exists on the 5' end of the hsp70 and hsp26 heat shock genes in uninduced cells and on the 5' end of at least some constutively expressed Drosophila genes. The main focus is on heat shock genes where release of polymerase beyond the pause site is rate-limiting in uninduced cells, and thus, is a potential target for the catalytic action of HSF during the heat shock response. The features of promoters that generate paused RNA polymerases will be identified by run-on assays performed with nuclei from uninduced transgenic fly lines containing altered hsp70 genes. The sites of pausing in vivo on native and altered heat shock genes will be examined at nucleotide resolution to determine whether the pause site is dictated by specific sequence elements or other features of the promoter. The release of paused polymerase in nuclei by addition of purified HSF and other nuclear fractions will be examined. Attempts will be made to establish an in vitro system that places a paused polymerase on an hsp70 gene template so that the mechanisms by which it is generated and released can be investigated.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM025232-17
Application #
2174401
Study Section
Molecular Biology Study Section (MBY)
Project Start
1978-04-01
Project End
1995-03-31
Budget Start
1994-04-01
Budget End
1995-03-31
Support Year
17
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

Name
Cornell University
Department
Biochemistry
Type
Schools of Arts and Sciences
DUNS #
City
Ithaca
State
NY
Country
United States
Zip Code
14850

  Publications

Booth, Gregory T; Parua, Pabitra K; Sansó, Miriam et al. (2018) Cdk9 regulates a promoter-proximal checkpoint to modulate RNA polymerase II elongation rate in fission yeast. Nat Commun 9:543
Tome, Jacob M; Tippens, Nathaniel D; Lis, John T (2018) Single-molecule nascent RNA sequencing identifies regulatory domain architecture at promoters and enhancers. Nat Genet 50:1533-1541
Chu, Tinyi; Rice, Edward J; Booth, Gregory T et al. (2018) Chromatin run-on and sequencing maps the transcriptional regulatory landscape of glioblastoma multiforme. Nat Genet 50:1553-1564
Vihervaara, Anniina; Duarte, Fabiana M; Lis, John T (2018) Molecular mechanisms driving transcriptional stress responses. Nat Rev Genet 19:385-397
Parua, Pabitra K; Booth, Gregory T; Sansó, Miriam et al. (2018) A Cdk9-PP1 switch regulates the elongation-termination transition of RNA polymerase II. Nature 558:460-464
Mahat, Dig B; Lis, John T (2017) Use of conditioned media is critical for studies of regulation in response to rapid heat shock. Cell Stress Chaperones 22:155-162
Boija, Ann; Mahat, Dig Bijay; Zare, Aman et al. (2017) CBP Regulates Recruitment and Release of Promoter-Proximal RNA Polymerase II. Mol Cell 68:491-503.e5
Vihervaara, Anniina; Mahat, Dig Bijay; Guertin, Michael J et al. (2017) Transcriptional response to stress is pre-wired by promoter and enhancer architecture. Nat Commun 8:255
Watters, Kyle E; Strobel, Eric J; Yu, Angela M et al. (2016) Cotranscriptional folding of a riboswitch at nucleotide resolution. Nat Struct Mol Biol 23:1124-1131
Booth, Gregory T; Wang, Isabel X; Cheung, Vivian G et al. (2016) Divergence of a conserved elongation factor and transcription regulation in budding and fission yeast. Genome Res 26:799-811

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